Enhancement of sensitivity of fluorophore mediated biosensing and bioimaging

ABSTRACT

A method of enhancing fluorescence emission in a fluorophore-mediated sensing, biosensing, imaging, and bioimaging. An example of biosensing is a fluorophore-mediated sandwich immunoassay with a 1° monoclonal antibody against a target analyte and a fluorophore-linked 2° monoclonal antibody, exposing the immunoassay to an enhancing agent, applying excitation light to the immunoassay, and measuring an emission signal from the immunoassay.

PRIORITY CLAIM

This application claims the benefit of U.S. Provisional Application Ser. No. 60/590,992, filed Jul. 26, 2004, under 35 U.S.C. §19.

FIELD OF THE INVENTION

A field of the invention is biosensing and bioimaging.

BACKGROUND OF THE INVENTION

Biomarkers used for disease diagnoses are usually present in bio-samples with a wide variety of other biomolecules, some of which are structurally homologous to the biomarkers themselves. In addition, the levels of the biomarkers in a sample are usually extremely low. Therefore, sensors to detect these biomolecules must be both very sensitive and specific.

Fluorophores have been valuable tools in biosensing/bioimaging for disease screening, diagnosis and monitoring. However, the low quantum yield (QY) of some of these fluorophores caused by non-radiative decay, especially by self-quenching, limits the effectiveness of these fluorophores in biosensing/bioimaging applications. Enhancement of the fluorescence can, therefore, improve the sensitivity of fluorophore-mediated biosensing and bioimaging.

SUMMARY OF THE INVENTION

Embodiments of the invention include a device and method for enhancing fluorescence emission in fluorophore-mediated biosensors. An exemplary method includes conducting a fluorophore-mediated sandwich immunoassay and exposing a flurophore-linked sandwich complex to an enhancing agent, such as a nanometal particle surrounded by a layer having a predetermined thickness (e.g., a self-assembled monolayer, surfactant or peptide), an organic, biocompatible solvent, or a combination of the nanometal particle with the self-assembled monolayer and the organic, biocompatible solvent. Another exemplary embodiment of the invention includes a biological sensor having enhanced fluorescence emission that includes an optical fiber having a fluorophore-mediated sandwich immunoassay disposed thereon, a chamber having at least one opening through which said fiber may extend, with an enhancing agent disposed in the chamber. The enhancing agent may be a nanometal particle a layer of predetermined thickness, an organic biocompatible solvent, or a combination of the nanometal particle having the layer of predetermined thickness, and the organic, biocompatible solvent.

BRIEF DESCRIPTION OF THE DRAWINGS

FIG. 1A is a schematic diagram comparing fluorescence emission between (I) conventional fiber optic immuno-sensing and (II) immuno-sensing using nanometal particles linked with self assembled monolayers according to an embodiment of the invention;

FIG. 1B is a schematic diagram illustrating the fluorescence measurement for free fluorophores in solution;

FIG. 2 is a schematic diagram illustrating an exemplary biosensor, Protein C Sensor, according to one embodiment of the invention;

FIG. 3 is a graph illustrating free fluorophore enhancement by 20 nm nanosilver particle-self-assembled monolayer 3 nm using fiber tip systems, where Cyanine 5 (CY5™) fluorophore concentration is fixed as 66 nM;

FIG. 4 is a graph illustrating BNP (a cardiac biomarker) sensing performance;

FIG. 5 is a graph illustrating the effect of solvents with various polarity on fluorescence enhancement of biosensing;

FIG. 6 is a graph illustrating the effect of nanogold particle-self-assembled monolayer, ethanol, or nanogold particle-self-assembled monolayer-ethanol combination on fluorescence enhancement;

FIG. 7 is a schematic diagram of the test for fluorescence enhancement in fiber optic immuno-biosensing: (a) the usual PC immuno sensing; (b) sensing with nanogold particle-self-assembled monolayer only; (c) sensing with ethanol only; and (d) sensing with both nanogold particle-self-assembled monolayer and ethanol;

FIG. 8 is a graph illustrating fluorescence enhancement using only a self-assembled monolayer (a) and (b), and fluorescence enhancement using a nanogold particle-self-assembled monolayer-ethanol (d) and (e);

FIG. 9 is a graph illustrating fluorescence enhancement of (a) Cyanine 5 (CY5™)-W; (b) nanogold particle-self-assembled monolayer-2 nm-Cyanine 5 (CY5™)-Water; and (c) nanogold particle-self-assembled monolayer-3 nm-AF647-W;

FIG. 10A is a graph illustrating the effect of self-assembled monolayer thickness on fluorescence enhancement for the free Cyanine 5 (CY5™)and the Cyanine 5 (CY5™) mediated PC sensing;

FIG. 10B is a graph illustrating the effect of nanogold particle size on the fluorescence enhancement for the free Cyanine 5 (CY5™) and the Cyanine 5 (CY5™) mediated PC sensing;

FIG. 10C is a graph illustrating the effect of nanogold particle size on the fluorescence enhancement for the free Cyanine 5 (CY5™) and the Cyanine 5 (CY5™) mediated PC sensing;

FIG. 11A is a graph illustrating the effect of nanogold particle-self-assembled monolayer, ethanol and NGPR on fluorescence enhancement of free Cyanine 5 (CY5™);

FIG. 11B is a graph illustrating the effect of ethanol and NGPRs with different self-assembled monolayers on fluorescence enhancement in PC sensing;

FIG. 12A is a graph illustrating the effect of NGPR on cardiac biomarker (cTnI) sensing; and

FIG. 12B is a graph illustrating the effect of NGPR on cardiac biomarker (BNP) sensing.

DETAILED DESCRIPTION OF THE PREFERRED EMBODIMENTS

Fluorescence of a fluorophore is normally limited by self-quenching of the free electrons in the fluorophore, thereby limiting the sensitivity of biosensors with which they are used. Embodiments of the invention reduce or eliminate this self-quenching, which enhances fluorescence emission of the fluorophore, thereby enhancing the ability to detect the presence of and quantify a target analyte. Fluorescence of some fluorophores and of fluorophore mediated biosensors is also enhanced significantly by biocompatible organic solvents. Devices and methods of the invention include exposing a fluorophore-mediated sandwich immunoassay to an enhancing agent, where the enhancing agent may be a nanometal particle having a layer of predetermined thickness, an organic, biocompatible solvent, or a combination of both a nanometal particle having a layer of predetermined thickness and an organic, biocompatible solvent.

Electrons of fluorophores that are normally involved in self-quenching upon photoexcitation may be coupled to strong surface plasmon polaritron fields of metallic nanoparticles, e.g., gold, silver, platinum and copper nanoparticles. Fluorescence can be maximized when a fluorophore is placed at a particular distance from the nanoparticle, wherein the particular distance may be empirically determined.

Embodiments of the invention exploit the surface plasmon polaritron fields of metallic nanoparticles, such as nanogold particles, nanosilver particles, nanoplatinum particles and nanocopper particles, for example, to enhance fluorescence. When plasmon rich, sharp metal tips or nanometal particles are placed at a particular distance from a fluorophore in accordance with the invention, they enhance the fluorescence by several fold, possibly by removing the cause of static or Foester quenching. This fluorescence enhancing effect can be artificially induced when a fluorophore is placed next to a metal particle treated with, for example, a self-assembled monolayer at a particular thickness. It is anticipated that the metal nanoparticle may be treated with a number of substances to obtain a layer having a predetermined thickness, such as a self-assembled monolayer, a surfactant, or a peptide, to name a few. The self-assembled monolayer will be discussed herein for purposes of illustration.

When placed at an appropriate, predetermined distance from a fluorophore, the metallic nanoparticles can effectively enhance fluorescence by transferring the free electrons of the fluorophore, electrons normally used for self-quenching, to the strong surface plasmon polaritron fields. If the metallic nanoparticle is placed too close to the fluorophore, the metallic nanoparticle extracts all electrons in the excited state from the fluorophore, including the ones for radiative emission. Alternatively, when the metallic nanoparticle is placed too far from the fluorophore, the surface plasmon polaritron fields may not reach the fluorophore, and there will be no effect on the resulting fluorescence intensity. However, when the appropriate predetermined distance is maintained between the metallic nanoparticle and the fluorophore via a predetermined mechanism, the fluorescence may be enhanced as the electrons normally used for self-quenching are transferred.

With application of embodiments of the invention, the sensitivity of the fluorophore mediated biosensor increases by several folds, which enables sensors with much higher sensitivity; increased accuracy diagnoses—fewer false positives or negatives; and minimization of the sensor size and assay time. Embodiments of the invention provide either fluorescence-enhancing nanometal particles, organic, biocompatible solvents, or a combination of both.

In embodiments using nanometal particles only, the invention contemplates using a variety of metallic nanoparticles, such as nanogold particles and nanosilver particles, nanoplatinum particles and nanocopper particles. However, for exemplary purposes, nanogold particles and nanosilver particles will be discussed herein for purposes of illustration. In a first preferred embodiment, a self-assembled monolayer of a predetermined thickness on the nanogold surface (“nanogold particle-self-assembled monolayer”) or nanosilver particle surface (“nanosilver particle-self-assembled monolayer”) is used to maintain the appropriate predetermined distance between the nanogold particle or nanosilver particle and the fluorophore. The self-assembled monolayer may include one of a plurality of molecules, preferably those water soluble, organic molecules with a thiol or amine terminal group in their structures, that may self-assemble onto the nanoparticles. For example, two such molecules are L-Glutathione and 16 mercaptohexadecanoic acid.

Other embodiments of the invention utilize one or more organic solvents to affect the fluorescence intensity in biosensing applications, even without exposure to nanometal particles having self-assembled monolayers. To maximize the fluorescence, embodiments of the invention include biocompatible organic solvents combined with metallic nanoparticles, such as nanogold particle reagents (NGPRs). Experiments have shown that organic solvents enhance fluorescence intensity. Without limiting the invention in any way, and only as a potential explanation of the mechanism for the enhancement, it is believed that organic solvents, such as ethanol, affect fluorescence intensity by 1) shifting the excitation/emission spectra of the fluorophore, 2) by the isomerization of the fluorophore, 3) by shrinking the fluorophore tagged proteins, or 4) by a combination of the three mechanisms. Preferred solvents include a solution that includes nanometal particles of less than 100 nm having self-assembled monolayers assembled thereon.

Still other embodiments include the use of one or more organic solvents in addition to maintaining a predetermined distance between the nanometal particle and the fluorophore using a self-assembled monolayer, where the effect of solvent on the level of fluorescence enhancement is additive. In one embodiment, use of the combination of nanogold particles having a self-assembled monolayer and a biocompatible solvent increase the signal of a fiber-optic biosensor as much as ten times, and can accurately quantify various cardiac markers at a tens of picomolar level.

Yet another preferred embodiment includes one or more organic solvents in combination with a SAM of a predetermined thickness to enhance fluorescence.

Embodiments of the invention are contemplated for sensing applications involving a virtually unlimited number of target analyte, especially proteins such as cardiac markers. For example, Cardiac Troponin I (cTnI) and Human B-type natriuretic peptide (BNP) are two cardiac markers that are very important for rapid and accurate heart attack diagnoses and prognosis. Protein C is a plasma anticoagulant and the accurate quantification can diagnose the genetic disorder, Protein C deficiency. The same principals may be used to diagnose various cancers.

Turning to FIG. 1A, for example, a first embodiment of the invention contemplates the use of nanogold particles of a particular size placed at a predetermined distance from a fluorophore in flurophore-mediated biosensing (immuno-optical protein C biosensor, for example) and bioimaging applications. While the size of the nanogold particles may vary to suit individual applications and are contemplated to include sizes ranging from 1 nm to 100 nm, nanogold particles ranging from 2 nm to 10 nm are optimal, preferably approximately 5 nm. A fluorophore-mediated immunoassay is conducted, with a 1° monoclonal antibody (1° Mab) 10 is immobilized on an optical fiber 12, such as a quartz fiber. The fiber may optionally include a beveled tip 14, polished to a predetermined angle, such as 45°. After exposure to a sample believed to include a target analyte 16 (e.g., protein C), a fluorophore-conjugated 2° monoclonal antibody (2° Mab) 18, such as Cyanine 5 (CY5™)-2° Mab, for example, binds the target analyte 16. As illustrated in box I, a fluorophore 19, which is represented by a star-shape, emits fluorescence upon the exposure to excitation light at a certain quantum yield. When the fluorophore-mediated sandwich complex is applied with nanogold particles-self-assembled monolayers 20, as illustrated in box II, the fluorescence is enhanced upon exposure to excitation light. The thickness of the self-assembled monolayers is an optimal thickness to maximize the enhancement, and in the instant embodiment, is contemplated to be between 1 nm and 10 nm, preferably between 1 nm and 3 nm, with approximately 2 nm providing maximum enhancement.

FIG. 1B illustrates an exemplary system in which a sensor may be used. The tip 14 of the fiber 12 is immersed in a buffer containing nanogold particles-self-assembled monolayer. At an end of the fiber 12 opposite the tip 14, the fiber is operably coupled to a fluorometer 24 that emits excitation light of a predetermined wavelength, and receives emission light from the fiber. The fluorometer 24 is preferably operably coupled to a computer 26 or other data acquisition device. Fluorescence emissions can accordingly be measured and the presence, absence and quantification of even small amounts of a target analyte may be ascertained.

By way of example only, a Protein C (PC) immuno-biosensor 28 for diagnosing a disease, PC deficiency, will be particularly described using FIG. 2 to illustrate. A distal end 29 of the quartz fiber 12 is tapered to increase evanescent signal retention and this portion of the fiber is encased in the chamber 22, which is a capillary sensor chamber. A surface of the fiber 12 is immobilized with 1° Mab 10 against PC. When a sample is injected into the chamber 22, the PC 30 binds specifically to 1° Mab 10 on the fiber surface with a high affinity. Then, the fiber 12 is preferably washed to remove unbound molecules. Next, the system is probed with another type of PC monoclonal antibodies that are tagged with a fluorophore 34, Cyanine 5 (CY5™)-2° Mab 36. After the reaction, excitation light, preferably of a wavelength of approximately 635 nm, is applied to the fiber 12. The Cyanine 5(CY5™)-2° Mab 36 bound to the PC 30 generate an emission signal of approximately 667 nm that is preferably interrogated by a long pass filter placed before a silicon detector (not shown). Then, the fluorescence intensity is correlated with the PC concentration. Since the 1° Mab 10 is covalently bound to the fiber 12, the fiber can be reused after adsorbed PC are eluted from the system using appropriate elution and regeneration buffers. The sample chamber 22 is very small (50-200 μl), requiring only a small sample volume per assay. The fluorescence generated from the immuno-optical biosensor is measured by the fluorometer 24.

A preferred embodiment uses nanosilver particles as an enhancer. While different sized nanosilver particles may be used, an approximately 20 nm sized nanosilver particles is illustrated, since it is the smallest commercially available nanosilver particle, though alternatively sized nanosilver particles are contemplated to suit individual applications as smaller particles become commercially available. FIG. 3 illustrates the enhancement of free fluorophore by nanosilver particles, and the mixture of the Cyanine 5 (CY5™) and 20 nm nanosilver particles with the Cyanine 5 (CY5™)/nanosilver particles ratio of 10/1 provided the highest enhancement of 23.3% compared to the pure Cyanine 5 (CY5™) solution.

Twenty nm nanosilver particles and the nanosilver particle reagent (NSPR) are also contemplated for use with the fluorophore-mediated BNP biosensor, as illustrated in FIG. 4. A 1.5 cm sensor was selected at 3 and 4 min incubation times for sample and 2° Mab, 1.2 cm/sec flow velocity, and a dye/nanosilver particles ratio of 20/1 and 2/1. The bottom line represents the sensing results without any enhancers. Compared to this control, 4%˜35% enhancements were observed by 20 nm nanosilver particles only, 100%˜114% enhancement by ethanol, the solvent only. The NSPR with fluorophore/nanosilver particle ratio of 20/1 provided 85%˜190% enhancement, while ratio of 2/1 provided the highest enhancement 185%˜245%. Therefore, these results confirm that the nanosilver particles and NSPR can also provide the fluorescence enhancements for free flourophore or fluorophore mediated biosensing.

Other embodiments of the instant invention include biocompatible solvents that enhance the fluorescence signal. Numerous solvents are anticipated, preferably those solvents that are biosensor compatible (i.e., not affecting the antibody affinity) and which do not prevent reusability of the fiber. While numerous organic solvents are contemplated for use with the invention, one preferred solvent is ethanol. FIG. 5 is a graph providing a comparison in fluorescence enhancement for several different solvents, including hexane, iso-propanol, n-butanol, THF, methanol, ethanol, DMSO and water. A 1.5 cm BNP sensor was used, with 1.2 cm/sec velocity, 3 and 4 min incubation times, 0.5 ng/ml BNP in plasma.

One particularly advantageous solvent is ethanol, which will be discussed for exemplary purposes. FIG. 6 illustrates the fluorescence enhancement when the fluorophore Cyanine 5 (CY5™) is mixed with (a) nanogold particle-self-assembled monolayer only; (b) ethanol only; and (c) nanogold particle-self-assembled monolayer and ethanol together. Experimental conditions included Cyanine 5 (CY5™) concentration of 0.066 μM, and a Cyanine 5 (CY5™)/nanogold particle ratio of 20/1. As can be seen in the figure, the enhancement by ethanol is even higher than that by nanogold particle-self-assembled monolayer, and when nanogold particle-self-assembled monolayer and ethanol are combined together the degree of the enhancement seems to be additive.

To illustrate with a specific example, the Protein C (PC) sensing system, a fluorophore such as either Cyanine 5 (CY5™) or ALEXA FLUORO™ fluorescent dye 647 (AF647) is conjugated with 2° Mab. The invention should not be construed as being limited to the fluorophores Cyanine 5 (CY5™) and AF647, as additional fluorophores are also contemplated for use with the invention. For example, ATTO 647, BODIPY™ 650/665 dye and DY-636 are additional potential fluorophores that may be used with the invention, to name a few. Cyanine 5 (CY5™) and AF647 were selected because they have very similar maximum excitation wavelengths (647 and 650 nm, respectively), but the quantum yield for AF647 is approximately twice of that for Cyanine 5 (CY5™). Therefore, the enhanced signal intensity for AF647 by nanogold particle-self-assembled monolayers is expected to be lower than that for Cyanine 5 (CY5™).

The intensity of the emission light generated from fluorophore-2° Mab quantifies the amount of PC in the sample. If the emission intensity by fluorophore-2° Mab is enhanced by even a few folds, then the sensor can become much more sensitive by increasing the signal to noise ratio (S/N ratio). Four different test cases are as shown in FIG. 7: (a) the control—a conventional PC sensing protocol; (b) applying only the nanogold particle-self-assembled monolayer after the completion of the Cyanine 5 (CY5™)-2° Mab reaction; (c) applying only ethanol; and (d) applying the mixture of the nanogold particle-self-assembled monolayer and ethanol. FIG. 8 illustrates the results of these cases of biosensing. In all cases, the enhancement in biosensing is several folds more than that with the free form of fluorophores. Also, the self-assembled monolayer thickness affects the degree of enhancement for both cases with only nanogold particle-self-assembled monolayer (in FIGS. 8, (a) and (b)), and nanogold particle-self-assembled monolayer-ethanol (in FIGS. 8, (d) and (e)), as in the free form. Again, the enhancement by nanogold particle-self-assembled monolayer and ethanol together shows the additive effect, e.g., as high as ten times of enhancement.

According to one embodiment of the invention, 5 nm sized nanogold particles are used. Nanogold particles are linked (treated) with two different lengths, 2 or 3 nm, of a self-assembled monolayer (SAM) and mixed with fluorophores, Cyanine 5 (CY5™) or AF647. Again, these two fluorophores were selected because they have very similar maximum excitation wavelengths.

The fluorescence from the mixture of fluorophore and nanogold particle-self-assembled monolayer was first measured using the tip of an optical fiber, as shown in FIG. 1B, and compared with that without nanogold particle-self-assembled monolayer. The fluorophore concentration in the buffer solution was 0.066 μM and the molar concentration ratio of nanogold particle-self-assembled monolayer to the fluorophores was 1:20. The ratio between the fluorophore and the gold particles affects the degree of enhancement and this ratio provides a clear enhancement. FIG. 9 summarizes the results of the level of the fluorescence enhancement when (a) Cyanine 5 (CY5™) is mixed with the NGPs linked with 3 nm SAM (SAM3 nm) in a water base buffer (W); (b) Cyanine 5 (CY5™) with the NGPs linked with 2 nm SAM (SAM2 nm) in the buffer; and AF647 is mixed with the NGPs linked with 3 nm SAM in the buffer. Two types of SAMs at thickness of ˜2 (MW=288) and ˜3 (MW=1701) nm, had been used. They are 16-Mercaptohexadecanoic acid and Tannic acid. The control is the fluorescence intensity from each dye molecules at the same concentration, without nanogold particle-self-assembled monolayers. From this figure, it is shown that the SAM thickness affects the level of the enhancement (2 nm enhances better). The tests also reveal possible enhancement by the fluorophore with a lower quantum yield (Cyanine 5 (CY5™)) is more than that of the fluorophore with higher one (AF647).

EXPERIMENTS AND RESULTS

Materials and Methods

Nanogold Particles-Self-Assembled Monolayer and NGPR Preparation

Nanogold colloids, which are nanogold particles (2, 5 and 10 nm) coated with tannic acid (surfactant, approximately 3 nm) were obtained. The thickness of a surfactant layer or self-assembled monolayer was theoretically estimated. L-Glutathione (approximately 1 nm) and 16 mercaptohexadecanoic acid (approximately 2 nm) were used as self-assembled monolayers. The self-assembled monolayer of L-glutathione or 16 mercaptohexadecanoic acid was linked on the surface of the nanogold particles by dissolving these molecules in distilled water or dimethyl sulfoxide; transferring them to the nanogold colloids; heating the mixture up to 70° C.; stirring them for 5 h; and purifying the products to eliminate the unreacted self-assembled monolayer molecules and replaced surfactant molecules. The NGPRs were produced by mixing the nanogold particles-self-assembled monolayers and the solvent to be tested.

Biosensor Preparation

Fluorophores, FLUOROLINK™ fluorescent product, Cyanine 5 (CY5™) and ALEXA FLUOR™ fluorescent dye 647 (AF647), were obtained. The Cyanine 5 (CY5™) or AF647 solution was prepared by dissolving the solid fluorophores in distilled water. A fluorometer with a long pass 670 nm filter inside and quartz fibers were used for sensors. Protein C and anti-PC monoclonal antibodies were obtained. Human B-type natriuretic peptide (BNP) and anti-BNP monoclonal antibodies were obtained. Cardiac Troponin I (cTnI) and anti-cTnI monoclonal antibodies were obtained. The PC sensor, PC samples, and fluorophore conjugated second antibody (fluorophore-2° Mab) were prepared.

Assay Protocol

The fluorescence of the free fluorophore in the phosphate buffer solution (PBS; control) or in the mixtures with nanogold particles-self-assembled monolayers or NGPRs was measured using a quartz fiber whose tip was polished at 45°. The fluorescence enhancement was also investigated with a fiber-optic PC sensor, which was developed for PC deficiency diagnosis. The sensor performs a fluorophore-mediated sandwich immunoassay on the sensor surface, and the fluorescence intensity is correlated with the PC concentration in blood plasma. Conventional assay protocol was used as a control: (1) sample injection and convective incubation, 0.5 min; (2) sensor washing and baseline measurement, 1 min.; (3) fluorophore-2° Mab injection and convective incubation, 2 min; (4) sensor washing and fluorescence measurement, 1 min.; (5) sensor regeneration, 1 min, and then the sensor is ready for the next assay. The signal used for the analyte quantification is the fluorescence measured in the step (4) subtracted by the baseline signal measured in the step (2).

For testing nanogold particles-self-assembled monolayers, solvents, or NGPRs, the protocol was modified to: (1′) nanogold particles-self-assembled monolayers, solvents or NGPRs injection and baseline measurement, 0.5 min; (2′) sensor washing, 0.5 min; (3′) sample injection and convective incubation, 0.5 min; (4′) sensor washing, 0.5 min; (5′) fluorophore-2° Mab injection and convective incubation, 2 min; (6′) sensor washing, 0.5 min; (7′) nanogold particles-self-assembled monolayers, solvents or NGPRs injection and fluorescence measurement, 0.5 min.; (8′) sensor washing and regeneration, 1.5 min. The fluorescence used for PC quantification is the value measured in the step (7′) subtracted by that measured in the step (1′).

Results and Discussion

Effects of the distance between a fluorophore and an NGP, and the NGP size on the fluorescence enhancement were studied. Since the concentration of the fluorophore and the NGP in a sample may also determine the distance, their concentrations were first adjusted to place them close enough to interact but not too crowded for quenching. The concentration ranges of the fluorophore and the nanogold particles used for this study were 10⁻⁸ to 10⁻⁷ and 10⁻¹⁰ to 10⁻⁷M, respectively. The fluorescence enhancement is defined as the increase in fluorescence by the enhancer divided by the fluorescence intensity without the enhancer.

The Effect of the Distance Between an NGP and a Fluorophore

Turning to FIGS. 10A-10C, in this study, the distance between a fluorophore and a nanogold particle was adjusted by the thickness of a self-assembled monolayer immobilized on the NGP surface. For this test, the nanogold particles size was kept constant at 5 nm. The thicknesses of the self-assembled monolayers tested were 1, 2 or 3 nm (L-glutathione, 16-mercaptohexadecanoic acid, and tannic acid, respectively). The nanogold particle-self-assembled monolayer was then applied to the free Cyanine 5 (CY5™) or the Cyanine 5 (CY5™) mediated PC biosensor and the fluorescence was measured (FIG. 10A). The ranges of the enhancement were 15˜44% for the free Cyanine 5 (CY5™) and 12˜215% for the PC sensing. The PC sensing results showed a trend qualitatively similar to those of the free fluorophore, but with several fold higher enhancements. For both cases, the self-assembled monolayer thickness of 2 nm provided the highest enhancement (44±4 and 25±8%, respectively). Although there were enhancements, 1 nm may have been too close to prevent reduction in radiative emission, and 3 nm may have been too far to transfer the electrons for effective enhancement.

The Effect of the Nanogold Particle Size

The effect of the nanogold particle size (2, 5 or 10 nm) was investigated at a constant SAM thickness of 3 nm (FIG. 10B). The enhancement for the free Cyanine 5 (CY5™) by 2, 5 and 10 nm nanogold particles were 42±5, 30±5, and 11±7%, respectively, showing a reduced enhancement as the nanogold particle size increased, possibly due to the differences in the surface plasmon polaritron field intensity for the nanogold particles of different size. For the PC biosensing, the enhancements were 115±10, 102±10, and 12±1%, respectively, showing a similar trend but much higher enhancements than those of the free fluorophore, as in the previous case. The higher enhancement in biosensing may be because free fluorophores suspended in solution interact with the nanogold particles in a three-dimensional space, not necessarily staying at the proximity of the fiber tip, while biosensing provides the sensor-surface-bound fluorophores for the nanogold particles to react.

Among the nanogold particle-self-assembled monolayers test (nanogold particle size of 2, 5 and 10 nm and self-assembled monolayer thickness of 1, 2 and 3 nm), 5 nm nanogold particles linked with 2 nm self-assembled monolayers (5 nm NGP-SAM 2 nm) were found to be the best enhancer.

The Effect of the Quantum Yield of a Fluorophore

Because it has been theorized that the fluorescence enhancement by nanogold particles is by retrieving the fluorescence that is normally self-quenched, it was expected that the amount of the enhanced fluorescence would depend upon the quantum yield (QY) of a fluorophore. To verify the theory, two fluorophores with the similar excitation/emission wavelengths, but with different QYs, were tested. Cyanine 5 (CY5™) (excitation/emission wavelengths: 649/670 nm) used in previous studies has a QY of 0.28. AF647 has excitation and emission wavelengths (649/666 nm) very similar to those of Cyanine 5's (CY5™), but has a QY of two times greater than that of Cyanine 5 (CY5™). The fluorescence enhancement of free AF647 by 5 nm nanogold particle-self-assembled monolayer 3 nm were studied and the results were compared with those of Cyanine 5's (CY5™). Free AF647 exhibited a significantly less enhancement (3±3%) than that of free Cy5 (30±5%). Also, in the AF647 mediated biosensing, as expected, there was very little enhancement. These results confirmed the hypothesis that the level of fluorescence enhancement by nanogold particles-self-assembled monolayers depends on the QY of the fluorophore.

The Solvent Effect

Various physical/chemical properties of organic solvents, such as viscosity, polarity, etc., may also affect the fluorescence. Three solvents which were considered to be not too harsh to biomolecules were ethanol, methanol and THF. These solvents were tested. When free Cyanine 5 (CY5™) was dissolved in ethanol, 92±4% enhancement was obtained, while signal reduction was exhibited in methanol and THF. This may be caused by the different solvent polarity and the behavior of hydrogen-bonds. However, 318±19, 166±21, and 434±32% of enhancements were achieved in PC sensing by ethanol, methanol and THF, respectively, implying the presence of other enhancing mechanisms for immobilized, protein-linked fluorophores. Although THF showed the highest enhancement in PC sensing, it affected the biosensor reusability (reduced from 7 to 4 times), possibly by permanently denaturing of 1° Mab molecules on the sensor surface. Ethanol appeared to be a desired enhancer because it did not affect the reusability. n-Butanol was found to be an even better enhancer. It also worked very well with AF647 both in the free form (90±4% enhancement) and the PC sensing (>100%), while the fluorescence of this fluorophore was not enhanced by nanogold particles-self-assembled monolayers (FIG. 10C). This indicates that the enhancement mechanism of solvents is different from that of the nanogold particles-self-assembled monolayers.

The Enhancement by NGPR

To maximize the enhancement effect, the two enhancers, the nanogold particles-self-assembled monolayers and the solvent, were mixed (NGPRs) and tested for their enhancement capacity. For 5 nm nanogold particles-self-assembled monolayers 3 nm mixed with ethanol, a 126±12% enhancement was demonstrated for free Cyanine 5 (CY5™), which appeared to be additively contributed from the enhancement by 5 nm nanogold particles-self-assembled monolayer 3 nm (30±5%) and by ethanol (94±9%) (FIG. 11A). Measurements were also performed for PC sensing with 5 nm nanogold particle of various self-assembled monolayer thickness, and for both free fluorophores and PC sensing the trend of the enhancement by these NGPRs was consistent by nanogold particles-self-assembled monolayers without ethanol (FIG. 10A). Quantitatively, the enhancement level for PC sensing with NGPRs was, again, several fold greater. For 5 nm nanogold particles-self-assembled monolayers 3 nm in ethanol, as an example, a 475±10% of enhancement was obtained, which was the combined effect by 5 nm nanogold particles-self-assembled monolayers 3 nm (102±10%) (FIG. 10A) and that by ethanol (318±31%). Ethanol is known to tightly fold proteins. Since the sensing principle of the immuno-biosensing is based on the retrieval of the fluorescent signals within the evanescent field, it was speculated that the ethanol may shrink the sandwich complex. As a result, fluorophore tagged 2° Mab may get closer to the sensor surface and the sensor retrieves more fluorescence per bound target biomarker. The protein structure change by ethanol is also known to be reversible and the application of ethanol, in fact, had no effect on the reusability of the PC sensor. PC sensing with 5 nm nanogold particles-self-assembled monolayers 2 nm in ethanol demonstrated the highest fluorescence enhancement, showing signal ten times stronger (898±28% enhancement) than that without any enhancers.

The Cardiac Marker Biosensing with NGPR

Fiber-optic biosensors are currently being developed to quantify cTnI and BNP in plasma, in their clinically significant ranges (31-310 and 26-260 pM), respectively. Because of their low target concentrations, without enhancers, the sensing performances of these two sensors were studied with 12 cm sensors and 10 min/10 min incubations. These markers were also measured with an NGPR (5 nm nanogold particles-self-assembled monolayers 2 nm in ethanol) by a 6 cm sensor with 5 min/5 min incubations (FIG. 12). Without enhancers, the 12 cm sensors produced very low signals. With the NGPR, a half sensor size, and a half assay time, 4 and 2.5 times of fluorescence enhancements were exhibited for the cTnI and BNP sensing, respectively, accurately quantifying cTnI and BNP.

Thus, fluorescence can be enhanced by well-designed nanogold particles-self-assembled monolayers, possibly by reducing self-quenching of fluorescence via the strong surface plasmon polaritron fields on the surface of a nanogold particle. This enhancement appears to be dependent on the nanogold particle size, the distance between a fluorophore and a nanogold particle, and the QY of a fluorophore. Some organic solvents also enhance the fluorescence significantly. Some biocompatible solvents, e.g. ethanol, are proven to be an optimal, fluorescence enhancer without affecting the reusability of biosensors. To maximize the enhancement effects NGPRs were developed by combining the nanogold particle-self assembled monolayer and the solvent. Among the NGPRs tested, the 5 nm nanogold particles-self-assembled monolayers at a thickness of 2 nm in ethanol was found to be the best enhancer. The mixture demonstrated an enhancement additive by the nanogold particle-self assembled monolayer and by the solvent. By utilizing NGPRs, accurate quantifications of cardiac markers at tens of picomolar level were achieved, enabling real-time heart attack diagnosis.

While specific embodiments of the present invention have been shown and described, it should be understood that other modifications, substitutions and alternatives are apparent to one of ordinary skill in the art. Such modifications, substitutions and alternatives can be made without departing from the spirit and scope of the invention. 

1. A biological sensor having enhanced fluorescence emission comprising: an optical fiber having a fluorophore-mediated biosensor disposed thereon; a chamber having at least one opening through which said fiber may extend; an enhancing agent disposed in said chamber; an excitation light source operably connected to said fiber; and a measuring device operably connected to said light source to measure fluorescence emission from the biosensor and said enhancing agent; wherein said enhancing agent comprises nanometal particles surrounded by a layer of a predetermined thickness, the layer providing a spacer separating the nanometal particles from the fluorophore that is sufficient to prevent fluorescence quenching said layer has a predetermined thickness of between 1 nm and 3 nm, and, said nanometal particles being dispersed within a solution including an organic, biocompatible solvent.
 2. The biological sensor of claim 1 wherein said fluorophore-mediated biosensor comprises a fluorophore-mediated sandwich immunoassay, said fluorophore-mediated sandwich immunoassay comprising a 1° monoclonal antibody bound to said fiber, a target analyte bound to said 1° monoclonal antibody, and a 2° monoclonal antibody bound to said target analyte.
 3. The biological sensor of claim 2 wherein said target analyte comprises at least one of Protein C, cTnI and BNP.
 4. The biological sensor of claim 1 wherein said layer comprises one of a self-assembled monolayer, a surfactants, and a peptides.
 5. The biological sensor of claim 1 wherein said nanometal particles are sized to be between 2 nm and 10 nm.
 6. The biological sensor of claim 1 wherein said nanometal particles are nanogold particles.
 7. The biological sensor of claim 1 wherein said enhancing agent further comprises at least one biocompatible organic solvent selected from the group consisting of n-butanol and ethanol.
 8. The biological sensor of claim 1, wherein said layer has a thickness of approximately 2 nm.
 9. A biological sensor having enhanced fluorescence emission comprising: an optical fiber having a fluorophore-mediated biosensor disposed thereon; a chamber having at least one opening through which said fiber may extend; an enhancing agent disposed in said chamber; an excitation light source operably connected to said fiber; and a measuring device operably connected to said light source to measure fluorescence emission from the biosensor and said enhancing agent; wherein said enhancing agent consists essentially of nanometal particles surrounded by a layer of a predetermined thickness and at least one organic, biocompatible solvent, the layer providing a spacer separating the nanometal particles from the fluorophore that is sufficient to prevent fluorescence quenching, and said layer has a predetermined thickness of between 1 nm and 3 nm, and; wherein the nanometal particles are dispersed within the at least one organic, biocompatible solvent.
 10. The biological sensor of claim 9, wherein said nanometal particles are nanogold particles.
 11. The biological sensor of claim 9, wherein said organic, biocompatible solvent is taken from the group consisting of n-butanol and ethanol. 